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来自疮痂链霉菌的一个编码假定致病因子的基因的克隆与表达。

Cloning and expression of a gene from Streptomyces scabies encoding a putative pathogenicity factor.

作者信息

Bukhalid R A, Loria R

机构信息

Department of Plant Pathology, Cornell University, Ithaca, New York 14853, USA.

出版信息

J Bacteriol. 1997 Dec;179(24):7776-83. doi: 10.1128/jb.179.24.7776-7783.1997.

Abstract

We cloned a 9.4-kb DNA fragment from Streptomyces scabies ATCC 41973 that allows the nonpathogen Streptomyces lividans 66 TK24 to necrotize and colonize potato tuber slices and produce scab-like symptoms on potato minitubers. Deletion analysis demonstrated that activity was conferred by a 1.6-kb DNA region. Sequence analysis of a 2.4-kb DNA fragment spanning the DNA region necessary for activity revealed three open reading frames (ORFs). The deduced amino acid sequence of ORF1, designated ORFtnp, showed high levels of identity with the first 233 amino acids of the putative transposases of the IS1164 elements from Rhodococcus rhodochrous (71%) and Mycobacterium bovis (68%), members of the Staphylococcus aureus IS256 family of transposases. No significant homologies to ORF2 and ORF3 were found in the nucleic acid and protein databases. ORFtnp is located 5' of ORF3. ORF2 is incomplete and is located 3' of ORF3. Subcloning of the individual ORFs demonstrated that ORF3, designated nec1, is sufficient for necrotizing activity in S. lividans 66 TK24. S. lividans 66 TK24 expressing nec1 does not produce thaxtomin A but produces an unidentified extracellular water-soluble compound that causes necrosis on potato tuber discs. The G+C content of nec1 suggests that it has moved horizontally from another genus. Southern analysis of ORFtnp and nec1 demonstrate that these genes are physically linked in Streptomyces strains, including S. scabies and Streptomyces acidiscabies strains, that are pathogenic on potato and that produce the phytotoxin thaxtomin A. These data suggest that nec1 may have been mobilized into S. scabies through a transposition event mediated by ORFtnp.

摘要

我们从疮痂链霉菌ATCC 41973中克隆了一个9.4 kb的DNA片段,该片段能使非致病菌变铅青链霉菌66 TK24对马铃薯块茎切片进行坏死性侵染并定殖,从而在微型薯上产生类似疮痂病的症状。缺失分析表明,活性由一个1.6 kb的DNA区域赋予。对跨越活性所需DNA区域的一个2.4 kb DNA片段进行序列分析,发现了三个开放阅读框(ORF)。ORF1的推导氨基酸序列命名为ORFtnp,与来自红球菌属的红平红球菌和牛分枝杆菌的IS1164元件推定转座酶的前233个氨基酸具有高度同源性(分别为71%和68%),它们属于金黄色葡萄球菌IS256转座酶家族成员。在核酸和蛋白质数据库中未发现与ORF2和ORF3有显著同源性。ORFtnp位于ORF3的5'端。ORF2不完整,位于ORF3的3'端。对各个ORF进行亚克隆表明,命名为nec1的ORF3足以在变铅青链霉菌66 TK24中产生坏死活性。表达nec1的变铅青链霉菌66 TK24不产生thaxtomin A,但产生一种未鉴定的细胞外水溶性化合物,该化合物会导致马铃薯块茎圆盘产生坏死。nec1的G+C含量表明它是从另一个属水平转移而来的。对ORFtnp和nec1的Southern分析表明,这些基因在包括疮痂链霉菌和酸疮痂链霉菌菌株在内的链霉菌菌株中物理连锁,这些菌株对马铃薯致病并产生植物毒素thaxtomin A。这些数据表明,nec1可能是通过由ORFtnp介导的转座事件被转移到疮痂链霉菌中的。

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